Literature DB >> 21189069

Matrigel improves functional properties of primary human salivary gland cells.

Ola M Maria1, Anthony Zeitouni, Olga Gologan, Simon D Tran.   

Abstract

Currently, there is no effective treatment available to patients with irreversible loss of functional salivary acini caused by Sjogren's syndrome or after radiotherapy for head and neck cancer. A tissue-engineered artificial salivary gland would help these patients. The graft cells for this device must establish tight junctions in addition to being of fluid-secretory nature. This study analyzed a graft source from human salivary glands (huSG) cultured on Matrigel. Cells were obtained from parotid and submandibular glands, expanded in vitro, and then plated on either Matrigel-coated (2 mg/mL) or uncoated culture dish. Immunohistochemistry, transmission electron microscopy, quantitative real-time-polymerase chain reaction, Western blot, and transepithelial electrical resistance were employed. On Matrigel, huSG cells adopted an acinar phenotype by forming three-dimensional acinar-like units (within 24 h of plating) as well as a monolayer of cells. On uncoated surfaces (plastic), huSG cells only formed monolayers of ductal cells. Both types of culture conditions allowed huSG cells to express tight junction proteins (claudin-1, -2, -3, -4; occludin; JAM-A; and ZO-1) and adequate transepithelial electrical resistance. Importantly, 99% of huSG cells on Matrigel expressed α-amylase and the water channel protein Aquaporin-5, as compared to <5% of huSG cells on plastic. Transmission electron microscopy confirmed an acinar phenotype with many secretory granules. Matrigel increased the secretion of α-amylase two to five folds into the media, downregulated certain salivary genes, and regulated the translation of acinar proteins. This three-dimensional in vitro serum-free cell culture method allows the organization and differentiation of huSG cells into salivary cells with an acinar phenotype.

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Year:  2011        PMID: 21189069     DOI: 10.1089/ten.TEA.2010.0297

Source DB:  PubMed          Journal:  Tissue Eng Part A        ISSN: 1937-3341            Impact factor:   3.845


  22 in total

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Review 2.  Current trends in salivary gland tight junctions.

Authors:  Olga J Baker
Journal:  Tissue Barriers       Date:  2016-03-10

3.  Silk fibroin scaffolds promote formation of the ex vivo niche for salivary gland epithelial cell growth, matrix formation, and retention of differentiated function.

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4.  Biomaterials-based strategies for salivary gland tissue regeneration.

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Journal:  Biomater Sci       Date:  2016-02-15       Impact factor: 6.843

5.  Encapsulation of Primary Salivary Gland Acinar Cell Clusters and Intercalated Ducts (AIDUCs) within Matrix Metalloproteinase (MMP)-Degradable Hydrogels to Maintain Tissue Structure and Function.

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Journal:  Adv Healthc Mater       Date:  2022-01-20       Impact factor: 9.933

6.  Implantable three-dimensional salivary spheroid assemblies demonstrate fluid and protein secretory responses to neurotransmitters.

Authors:  Swati Pradhan-Bhatt; Daniel A Harrington; Randall L Duncan; Xinqiao Jia; Robert L Witt; Mary C Farach-Carson
Journal:  Tissue Eng Part A       Date:  2013-05-10       Impact factor: 3.845

Review 7.  Comparing human and mouse salivary glands: A practice guide for salivary researchers.

Authors:  C L Maruyama; M M Monroe; J P Hunt; L Buchmann; O J Baker
Journal:  Oral Dis       Date:  2018-04-24       Impact factor: 3.511

Review 8.  Current cell models for bioengineering a salivary gland: a mini-review of emerging technologies.

Authors:  J Nelson; K Manzella; O J Baker
Journal:  Oral Dis       Date:  2012-07-18       Impact factor: 3.511

9.  An in vitro culture system for long-term expansion of epithelial and mesenchymal salivary gland cells: role of TGF-β1 in salivary gland epithelial and mesenchymal differentiation.

Authors:  Kajohnkiart Janebodin; Worakanya Buranaphatthana; Nicholas Ieronimakis; Aislinn L Hays; Morayma Reyes
Journal:  Biomed Res Int       Date:  2013-06-09       Impact factor: 3.411

10.  Three-Dimensional Culture of Ameloblast-Originated HAT-7 Cells for Functional Modeling of Defective Tooth Enamel Formation.

Authors:  Anna Földes; Thanyaporn Sang-Ngoen; Kristóf Kádár; Róbert Rácz; Ákos Zsembery; Pamela DenBesten; Martin C Steward; Gábor Varga
Journal:  Front Pharmacol       Date:  2021-06-02       Impact factor: 5.810

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